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Preventing swarm detection in extracellular vesicle flow cytometry: a clinically applicable procedure

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DOI: 10.1016/j.rpth.2023.100171

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biomarkers; exosomes; extracellular vesicles; flow cytometry; plasma

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A practical procedure was developed to determine the optimal sample dilution for plasma in order to prevent swarm detection and maintain significant particle counts in clinical research studies. The optimal dilution factor was found to be ≤1.1×10^2-fold, and the count rate should be <1.1×10^4 events center dot s^(-1).
Background: Flow cytometry is commonly used to detect cell-derived extracellular vesicles in body fluids such as blood plasma. However, continuous and simultaneous illumination of multiple particles at or below the detection limit may result in the detection of a single event. This phenomenon is called swarm detection and leads to incorrect particle concentration measurements. To prevent swarm detection, sample dilution is recommended. Since the concentration of particles differs between plasma samples, finding the optimal sample dilution requires dilution series of all samples, which is unfeasible in clinical routine. Objectives: Here we developed a practical procedure to find the optimal sample dilution of plasma for extracellular vesicle flow cytometry measurements in clinical research studies. Methods: Dilution series of 5 plasma samples were measured with flow cytometry (Apogee A60-Micro), triggered on side scatter. The total particle concentration between these plasma samples ranged from 2.5 x 10(9) to 2.1 x 10(11) mL(-1). Results: Swarm detection was absent in plasma samples when diluted =1.1 x 10(3)-fold or at particle count rates <3.0 x 10(3) events center dot s(-1). Application of either one of these criteria, however, resulted in insignificant particle counts in most samples. The best approach to prevent swarm detection while maintaining significant particle counts was by combining minimal dilution with maximum count rate. Conclusion: To prevent swarm detection in a series of clinical samples, the measurement count rate of a single diluted plasma sample can be used to determine the optimal dilution factor. For our samples, flow cytometer, and settings, the optimal dilution factor is = 1.1 x 10(2) -fold, while the count rate is <1.1 x 10(4) events center dot s(-1)

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